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Carotenoids and Antioxidant Enzymes as Biomarkers of the Impact of Heavy Metals in food Chain

Vangelis Andrianos1*, Vasiliki Stoikou1, Konstantina Tsikrika3, Dimitra Lamprou1, Sotiris Stasinos1, Charalampos Proestos1, and Ioannis Zabetakis1,2

1Laboratory  of  Food  Chemistry,  Department  of  Chemistry,  University  of   Athens,  15771,  Athens,  Greece
2Department of Life Sciences, University of Limerick, Limerick, Ireland
3School of Science, Engineering & Technology, Abertay University, Dundee, Scotland.

Corresponding Author Email: vandrianos@chem.uoa.gr

DOI : https://dx.doi.org/10.12944/CRNFSJ.4.Special-Issue1.02

Article Publishing History

Published Online: 26-02-2016

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Abstract:

Antioxidant enzymes (catalase and peroxidase) and carotenoids lutein and  β-carotene are often used as biomarkers of metal contamination of water  and agricultural soils. In this study, the effects of heavy metals present in  irrigation water on the aforementioned carotenoids of potatoes Solanum  tuberosum L. and carrots Daucus carota L., cultivated in a greenhouse and irrigated with a water solution including different levels of Cr(VI) and Ni(II) were investigated. These results were compared to the levels of the same metabolites that had been assessed in market-available potato and carrot samples. The findings indicated that the levels of the examined metabolites on the treated with Cr and Ni samples, resemble the levels of the same parameters in the market samples, originating from polluted areas. Therefore, the antioxidant enzymes, catalase and peroxidase, and the carotenoids,  lutein and β-carotene, could be handled as indicators of heavy metal pollution.

Keywords:

Heavy metals; Food tubers; Antioxidant enzymes; Carotenoids; Biomarkers

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Andrianos V, Stoikou V, Tsikrika K, Lamprou D, Stasinos S, Proestos C, Zabetakis I. Carotenoids and Antioxidant Enzymes as Biomarkers of the Impact of Heavy Metals in food Chain. Curr Res Nutr Food Sci 2016;4(Special Issue Carotenoids March 2016). doi : http://dx.doi.org/10.12944/CRNFSJ.4.Special-Issue1.02


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Andrianos V, Stoikou V, Tsikrika K, Lamprou D, Stasinos S, Proestos C, Zabetakis I. Carotenoids and Antioxidant Enzymes as Biomarkers of the Impact of Heavy Metals in food Chain. Curr Res Nutr Food Sci 2016;4(Special Issue Carotenoids March 2016). http://www.foodandnutritionjournal.org/?p=2247


Introduction

Soil and water quality have a direct impact on the quality of our environment and consequently on our nutrition and health.1 Environmental pollution due to anthropogenic operations such as sewage sludge, mining, industrial and domestic wastewater or excessive application of fertilizers and  pesticides may lead to bioaccumulation of heavy metals in crops2 and thus to serious cross-contamination of the food chain.3 Heavy metal contamination of crops, such as potatoes and carrots, which are principal components of our daily diet,  is a matter of great concern, as their consumption may result in accumulation of risk elements in the human body which can cause serious health  problems.4 However, the US and EU legislation for heavy metals in food is inadequate (i.e. only four heavy metals are regulated under current EU legislation, EC 1881/2006); whereas the respective legal limits for water are harsh.5

The use of biomarkers as indicators of the pollutant effect on an ecosystem has been widely studied in order to gain knowledge on the physiological or biochemical response of an organism to pollutant exposure.6,7 Measurements of biochemical responses to pollutants may serve  as early signals of biologically significant toxic exposure given that toxic effects tend to appear at the subcellular level before appearing at higher  levels of biological  organisms.8

Biomarkers, such as enzyme activity and carotenoid levels could be used  as indicators of the oxidative stress caused by heavy metal pollution. Therefore their assessment is more relevant biologically, when compared to trace element analysis. Furthermore, the analysis of these secondary metabolites has three distinct advantages, being swift and of low cost and not requiring expensive instrumentation as opposed to the techniques that are commonly used for the determination of heavy metal concentrations.

Previous studies of our team investigated the cross-contamination of the food chain caused by the environmental pollution in Asopos land (one of the biggest industrial areas of central Greece) by heavy metals; the levels of Ni and Cr were significantly higher in crops from Asopos area than in plants grown in areas besides water-bed pollution (control samples).3,5 Another study of our team on the effects of these trace elements on the carotenoids and the antioxidant  activity (DPPH) of carrots, potatoes and onions (Allium cepa L.) showed that the levels of β-carotene in carrots and the levels of lutein in potatoes from the Asopos area were significantly lower as opposed to the control samples.9 These two researches were the incentive of a greenhouse experiment, conducted by our team where the open-field  irrigation  conditions of Asopos area and Messapia region (Evia, Greece) were simulated. Both these regions have considerable levels of Cr and Ni in the underground water. The uptake of these heavy metals by carrots, potatoes and onions was studied and the resulting cross-contamination by the irrigation water of the potatoes and onions was screened, but no cross-contamination was observed for carrots.10

In the present study, our scope was three-fold: 1) to examine the effects of  Cr(VI) and Ni(II) in irrigation water on the carotenoid content (lutein and β-carotene) and the activities of antioxidant enzymes (catalase and peroxidase) in potatoes and carrots, cultivated in a greenhouse whilst being irrigated with Cr(VI) and Ni(II) contaminated water, 2) to compare the results of 10 to findings in the respective crops, bought from the local market and developed in areas with or without water-bed pollution and 3) to investigate the possibility of using the aforementioned parameters as biomarkers of heavy metal pollution.

Materials and Methods

Experimental Design

Plants’ cultivation in a greenhouse 

For  the  purposes  of  this  study,  potatoes  and  carrots  were  planted  in  a greenhouse (Harokopio University, Athens, Greece),  at which the installation  had four lines with irrigated water  (i.e. four 300 L plastic tanks, four pumps, and  four series of two tubs per series) was used. The cultivation duration was four months (September 2012 to January 2013). The four irrigation lines contained various levels of Cr(VI) and Ni(II), as follows: 0 μg L-1 (control),  100 μg L-1, 250 μg L-1 and 1,000 μg L-1. The solutions were prepared by solid K2Cr2O7 and NiCl2.6H2O, diluted in tap water. All the plants were fertilized once every month (15N-30P-15K fertilizer, 2-4 g dry solids/plant diluted in water, depending on plant size) and irrigated every 3-10 days (depending on soil humidity). They were also supervised by a professional agriculturalist. The amounts of the main characteristics of control (clean) water were: pH=8.3, turbidity=7.6 NTU, EC=295 μS cm-1, TDS=156 mg l-1, Na=4.6 mg l-1, K=0.8 mg l-1, Pb=0.3 mg l-1, Hg=0 mg l-1, Cd=0 mg l-1, Cr=0 mg l-1.

 Figure 1.Picture of the Experimental Design. Figure 1: Picture of the Experimental Design.  

Click here to View figure

 

Market Samples

Commercially available samples (potatoes and carrots, five different samples of each vegetable) originating from Greece and from other European countries (Holland and Cyprus) were obtained from supermarkets in Athens, Greece, the same period, when the greenhouse’s vegetables were analyzed.

Enzyme assay

Materials

The materials used for catalase and peroxidase assay were potassium  phosphate monobasic (KH2PO4), potassium phosphate dibasic (K2HPO4), ethylenediaminetetraacetic acid (EDTA), guaiacol, hydrogen peroxide (H2O2),  plastic and quartz cuvettes (all from Sigma-Aldrich, Germany) and double  distilled water (DDW).

Enzyme extraction      

Potatoes and carrots were cut into small pieces and homogenized with phosphate buffer (50 mM, pH 7.0) containing 1 mM of EDTA. The homogenate got filtered through and the obtained extract was centrifuged at 7000 × g for 20 minutes at 4°C. The clear supernatant was kept at 0-4°C in 5 mL vials and was suitably thawed before the enzyme analysis.11

Enzyme analysis

Catalase (CAT E.C.1.11.1.6) activity (ΔΑ240 min-1 g-1 FW) assay was based on the absorbance at 240 nm on the UV spectrophotometer. The decrease in absorbance was recorded over a period as described previously.12 A complete reaction mixture was including 1.5 mL of 100 mM potassium phosphate buffer (pH 7.0), 0.5 mL of 75 mM H2O2, 0.2 mL of enzyme extract and 0.8 mL of DDW, in quartz cuvettes.

Peroxidase (POX E.C.1.11.1.7) activity (ΔΑ470 min-1 g-1 FW) was assayed as an increase in optical density because of the oxidation of guaiacol to tetraguaiacol13. The complete reaction mixture contained 1.0 ml of 100 mM potassium phosphate buffer (pH 6.1), 0.5 ml of 96 mM guaiacol, 0.5 mL of 12 mM H2O2, 0.1 ml of enzyme extract and 0.4 ml of double distilled water (DDW). The enzyme activity was measured at 470 nm, in plastic cuvettes, for 1 min on a UV spectrophotometer.

Every plant sample was analysed in triplicate.

High Performance Liquid Chromatography (HPLC) Assay   

Materials

All materials were obtained from Merck, Germany except of lutein which was obtained from Extrasynthese, France and β-carotene which were obtained from Fluka, UK.

Sample Preparation

All plant samples were washed thoroughly with double distilled water (DDW) and were peeled and carved afterwards. Then, they were ground to obtain a thin powder using a food processor with stainless steel cutters and then stored at –15 °C before the assay. The extraction of carotenoids was performed as described before14 with minor modifications. More specifically, carotenoids were released from the powdered samples (5g) by adding 0.5 g of magnesium carbonate and 25 mL of 50:50 methanol:tetrahydrofuran (THF). The crude suspensions were centrifuged at 6000 × g at 4 °C for 10 min (Sorvall RC-5B Refrigerated Superspeed Centrifuge, Du Pont Instruments). The process was repeated until the extracting solvent was colorless and the extract was vacuum filtered thereafter. The filtrates were then concentrated using a rotary evaporator apparatus (Heidolph Laborota 4000 eco/WB/G1) and transferred to a 25 mL volumetric flask, while carrot extracts were diluted to a known volume with methanol so that THF levels were less than 10% of the entire solution. Before the injection into the HPLC analysis system, all samples were filtered through a 0.45 μm filter. All analyses were done in triplicate.

Preparation of Calibration Curves

Five mg of lutein were dissolved in 100 mL reagent alcohol containing 30 mg L-1 butylated hydroxytoluene (BHT), while 5 mg of β-carotene were dissolved in 10 mL THF (1 l of THF previously stabilized with 250 mL BHT) and then diluted to 100 mL with reagent alcohol. Full standard curves were constructed with five different concentrations for each carotenoid. The concentrations for the lutein standards were from 0.01 to 0.16 mg L-1, while the β-carotene concentrations were from 0.5 to 10.0 mg L-1, as described before.15 All analyses of standard solutions were performed in triplicate.

The calibration curves obtained (y being the peak area, x being the concentration of the standard compound in mg L-1) were y = 1236560.31 x + 3574.21 with R2 = 0.9999 for lutein and y = 1559668.43 x – 165770.72  with R2 = 0.9986 for β-carotene.

HPLC Analysis

The HPLC apparatus consisted of an Agilent SERIES 1100, equipped with a Variable Wavelength UV-Vis detector and an integrator Agilent 3395. A 50 μl loop was used. All solvents had purity of HPLC grade. The mobile phase was a binary mixture of methanol : acetonitrile  (85:15, v/v). The column was a C18 Zorbax SB (4.6 × 250 mm, 5 μm). The column was kept at room temperature (20 °C) and the flow rate was 1.5 ml min-1. The detection wavelength was 450 nm.

Statistical methodology

All analyses were carried out in triplicate and the results were statistically edited using IBM SPSS.19

The Mann-Whitney non-parametric test was applied for the “two by two”  comparisons between the groups of plants irrigated with different concentrations of heavy metals (Cr, Ni) in relation to their metabolites (catalase, peroxidase, lutein and β-carotene).

Therefore, each group of plants irrigated with the same metals concentrations (plants grown in the same tub or plants grown in the same geographical area) was compared with each and every other group of plants irrigated with other concentrations (e.g. 0 and 100 μg/l, 0 and 250 μg/l, Naxos and 0 μg/l, etc.) to find out if there were statistically significantly differences in the metabolites of the different groups. The comparisons between the groups of plants were based on median values of metabolites. The choice of the median values, instead of mean values, was made because, in many occasions, the distributions of values diverged from the normal distribution.

Results

For the total growing season (September 2012 – January 2013) each tuber was irrigated with approximately 40 L of water with Cr(VI) and Ni(II)  concentrations varying from 0 to 1000 μg L-1. The range of the metal  concentrations was chosen in order to resemble the concentration levels of  Cr(VI) and Ni(II) that have been detected in the underground waters of Asopos  area and Messapia and thus, to simulate as close as possible these open-field cultivation conditions.3 The total mass of Cr(VI) and Ni(II) added in each  tub, for the irrigation watering line of 0, 100, 250, and 1,000 μg L-1, was 0,  4,000,  10,000, and 40,000 μg, respectively. No symptoms of toxicity were observed in any plant. The antioxidant enzyme and the carotenoid response of potato and carrot samples to heavy metal treatment are described in Table 1, while the results of statistical analysis are shown in Table 2.

Table 1: Levels of catalase, peroxidase, lutein and β-carotene(Levels of catalase and peroxidase in ΔΑ g-1 min-1 fresh  weight, lutein and  β-carotene in μg g-1  fresh  weight. Potato and carrot samples irrigated with water solution containing Cr(VI) and  Ni(II) in concentrations ranging from 0 to 1000 μg L-1)

Parameter

0 μg L-1.

100 μg L-1.

250 μg L-1.

1000 μg L-1.

Catalase (p)a

0.160 ± 0.047

0.167 ± 0.029

0.138 ± 0.097

0.162 ± 0.031

Peroxidase (p)a

2.075 ± 0.171

7.125 ± 1.769

3.625 ± 2.42

4.350 ± 0.645

Lutein (p)a

0.080  ± 0.001

0.312 ± 0.049

0.024 ± 0.014

nd

Catalase (c)b

0.088 ± 0.024

0.054 ± 0.014

0.046 ± 0.027

0.052 ± 0.004

Peroxidase (c)b

0.675 ± 0.126

0.275 ± 0,096

0.775 ± 0.299

0.325 ± 0.126

Lutein (c)b

6.117 ± 2.620

4.608 ± 0,525

6.172 ± 1.450

2.015 ± 0.325

β-Carotene (c)b

38.603 ± 12.080

57.588 ± 14,710

58.895 ± 34.320

31.598 ± 7.290

Results are expressed as mean ± standard deviation (n=3).

a: potato  samples

b: carrot  samples

nd: not  detected

Table 2: “Two by two” comparisons of the enzyme activity and carotenoid content of potatoes and carrots 

μg L-1 Cr & Ni

p-value

Catalase

Peroxidase

Lutein

β-Carotene

Potatoes

Carrots

Potatoes

Carrots

Potatoes

Carrots

Carrots

0

100

0.886

0.029a

0.029a

0.029a

0.029a

0.229

0.629

250

0.686

0.057b

0.343

0.686

0.029a

0.629

0.400

1000

0.606

0.029a

0.029a

0.029a

0.057b

0.057b

100

250

0.343

1.000

0.057b

0.029a

0.029a

0.114

0.686

1000

0.686

1.000

0.057b

0.686

0.029a

0.029a

250

1000

0.486

0.629

0.886

0.057

0.029a

0.029a

a: statistically significant (p<0.05) (Mann-Whitney non parametric test)

 

b: marginally significant (0.05<p<0.1) (Mann-Whitney  non parametric test)

CAT activity in potato samples did not show any statistically significant differences, whereas POX activity has increased statistically significantly in  potato samples irrigated with water containing 100 μg L-1 (+243.4  percent  in  median value) and 1000 μg L-1 (+109.6 percent in median value) of Cr(VI)  and Ni(II) as opposed to control samples. A marginally significant decrease

was observed in potato crops irrigated with water containing 250 μg L-1 (-56.1  percent in median value) and 1000  μg L-1 (-38.9 percent in median value) of  Cr(VI) and Ni(II) in respect to potato samples irrigated with 100 μg L-1.

The increased activity of POX suggests strong induction of oxidative stress as antioxidant enzymes constitute part of the detoxification mechanisms in plants.16 These high levels of the antioxidant enzyme activity may have been an immediate reply to the generation of superoxide radicals by Cr-induced blockage of the electron transport chain in the mitochondria.17

CAT activity in carrot samples irrigated with water containing 100 μg L-1  and 1000 μg L-1 Cr(VI) and Ni(II) decreased statistically significantly (-38.6  percent and -47.7 percent in median value, respectively) as correlated to the  control ones. POX activity in carrot crops irrigated with water containing 100 μg L-1 Cr(VI) and Ni(II) decreased statistically significantly as compared to the control samples and the ones irrigated with water containing 250 μg L-1 Cr(VI) and Ni(II) (-59.2 percent in median value and -64.5 percent in median value, respectively). A statistically significant decrease was also noticed in the carrot  crops irrigated with water containing 1000 μg L-1 in respect to the control ones  (-51.8 percent in median value), whereas the decrease was marginally  significant as compared to the carrot samples irrigated with water containing  250 μg L-1 Cr(VI) and Ni(II) (-58.1 percent in median value).

Low CAT and POX activities result in an increase of H2O2 levels, causing oxidative stress, inactivation of CAT and finally blockage of the synthesis of new enzyme.18 CAT is naturally present in peroxisomes, where it catalyzes the disintegration of the H2O2 produced during photorespiration.19 A previous study on carrots treated with excess Cr found decreased CAT activity in carrot leaves,20 possibly as a result of the absolute or partial substitution of Fe from active sites or due to low levels of Fe in leaves inhibiting the embodiment of Fe in porphyrin of the enzyme.21-23 Furthermore, the decreased activity of POX may have occurred as a consequence to peroxidative damages of the thylakoid membrane.24

Lutein content in potato crops irrigated with water containing 100 μg L-1 Cr(VI) and Ni(II) increased statistically significantly as opposed to the control ones (+290 percent in median value), while lutein levels in potato samples irrigated with water containing 250 μg L-1 Cr(VI) and Ni(II) decreased statistically significantly as compared to the control samples and the ones polluted with water containing 100  μg L-1 Cr(VI) and Ni(II) (-70 percent in median value and -92.3 percent in median value, respectively). Lutein levels in potato crops irrigated with water including 1000 μg L-1 Cr(VI) and Ni(II) were not detectable.

β-Carotene and lutein levels in carrot crops irrigated with water containing  1000 μg L-1 Cr(VI) and Ni(II) decreased marginally significantly as opposed to  the control ones (-18.1 percent, in median value and -67 percent in median value, respectively), whereas the decrease was statistically significant in  respect to the β-carotene and lutein content of the carrot samples irrigated  with water containing 100 μg L-1 Cr(VI) and Ni(II) (-45.1 percent in median  value and -56.3 percent in median value, respectively) and 250 μg L-1 Cr(VI) and Ni(II) (-46.3 percent in median value and -67.4 percent in median value, respectively).

Chromium toxicity can cause metabolic disturbances such as transitions in pigment production, augmentation of metabolite production (ascorbic acid, glutathione) and the generation of new metabolites as a reinforcement of the detoxification mechanism of the plant,17 while nickel can provoke suppression in growth and reduction of the Fe levels.24 Even if an amount of these trace elements can be filtered or rejected through the plant root tissues, higher levels of heavy metals in the soil are affiliated to virulent effects.25

As has been observed earlier for potato and carrot crops grown in Asopos region (where the underground waters are contaminated by heavy metals), heavy metals may induce the biosynthesis of lutein and β-carotene. Lutein and β-carotene levels in Asopos potatoes and carrots, respectively, decreased as compared to the carotenoid levels in the control samples, suggesting an impact of heavy metals in carotenoid metabolic pathway.9

The results of carotenoid and antioxidant enzymes analysis of potato and carrot market samples are shown in tables 3 and 4, while the results of the statistical analysis of the samples are visible in the tables 5 and 6.

Table 3: Catalase, peroxidase and lutein levels in potato market samples originating from Greece and Cyprus.  (Levels of catalase and peroxidase in ΔΑ g-1 min-1 fresh weight and lutein in μg g-1 fresh weight)

Parameter

Achaia (GR)

Evia (GR)

Cyprus

Orhomenos BIO(GR)

Naxos (GR)

Catalase

0.131 ± 0.016

0.167 ± 0.056

0.037 ± 0.006

0.127 ± 0.038

0.041 ± 0.014

Peroxidase

5.180 ± 0.075

8.600 ± 0.351

6.650 ± 0.050

4.150 ± 0.350

3.930 ± 0.225

Lutein

0.033 ± 0.029

nd

Nd

0.245 ± 0.102

0.041 ± 0.011

Results are expressed as mean ± standard deviations (n=3).
nd: not  detected

Table 4: Catalase, peroxidase, lutein and β-carotene levels in carrot market samples originating from Greece and Holland.

(Levels of catalase and peroxidase in ΔΑ g-1 min-1 fresh weight and lutein and β-carotene in  μg g-1 fresh weight).

Parameter

Evia (GR)

Avlonas (GR)

Holland BIO

Viotia (GR)

Marathon(GR)

Catalase

0.081 ± 0.012

0.037 ± 0.025

0.104 ± 0.073

0.008 ± 0.002

0.087 ± 0.048

Peroxidase

0.400 ± 0.125

0.400 ± 0.050

0.175 ± 0.025

0.025 ± 0.075

0.250 ± 0.100

Lutein

6.600 ± 1.000

5.610 ± 1.980

7.650 ± 1.912

5.150 ± 0.345

5.490 ± 0.139

β-Carotene

52.310 ± 0,568

64.660 ± 16.165

59.500 ± 14.875

52.500 ± 0.490

55.150 ± 11.878

Results are expressed as mean ± standard deviations (n=3).

Table 5: “Two by two” comparisons of the enzyme activity and the carotenoid content in potatoes.

Potato  Market samples  from  Greek  areas  and Cyprus

μg L-1 Cr & Ni

Catalase

(p-value)

Peroxidase

(p-value)

Lutein

(p-value)

Achaia (GR)

0

0.486

0.029a

0.057b

100

0.343

0.343

0.057b

250

1.000

0.343

1.000

1000

0.486

0.200

Evia (GR)

0

0.343

0.029a

100

0.886

0.343

250

0.686

0.029a

1000

0.686

0.029a

 

0

0.029a

0.029a

Cyprus

100

0.029a

0.686

250

0.029a

0.057b

1000

0.029a

0.029a

Orhomenos BIO (GR)

0

0.686

0.029a

0.057b

100

0.343

0.029a

0.400

250

0.886

1.000

0.057b

1000

0.486

1.000

Naxos (GR)

0

0.029a

0.029a

0.057b

100

0.029a

0.029a

1.000

250

0.057b

1.000

0.057b

1000

0.029a

0.200

a:  statistically  significant  difference  (p<0.05)  (Mann-Whitney  non  parametric  test)

 

b:  marginally  signif 

Table 6: “Two by two” comparisons of the enzyme activity and the carotenoid content in carrots.

Carrot  Market samples  from Greek  areas and  Holland

μg L-1 Cr & Ni

Catalase

(p-value)

Peroxidase

(p-value)

Lutein

(p-value)

β-Carotene

(p-value)

Evia (GR)

0

0.868

0.057b

0.343

0.114

100

0.114

0.200

0.057b

0.343

250

0.114

0.114

1.000

0.343

1000

0.057b

0.486

0.029a

0.029a

Marathon (GR)

0

0.686

0.029a

0.343

0.114

100

0.686

0.886

0.114

1.000

250

0.343

0.029a

0.486

0.686

1000

0.200

0.486

0.029a

0.029a

 

0

0.886

0.029a

0.724

0.886

Holland BIO

100

0.343

0.200

0.686

0.057b

250

0.029a

0.029a

0.400

0.486

1000

0.200

0.114

0.343

0.029a

Avlonas (GR)

0

0.057b

0.029a

0.686

0.200

100

0.486

0.114

0.343

0.343

250

1.000

0.114

1.000

0.686

1000

0.343

0.343

0.343

0.343

Viotia (GR)

0

0.029a

0.029a

0.400

0.114

100

0.029a

0.486

0.629

0.343

250

0.200

0.029a

0.229

0.343

1000

0.029a

0.343

0.057b

0.029a

a:  statistically  significant  difference  (p<0.05)  (Mann-Whitney  non  parametric  test)

b:  marginally  significant  difference  (0.05<p<0.1)  (Mann-Whitney  non  parametric  test)

Given the statistically significant and the marginally significant differences which have emerged from the comparison between the same biomarkers in the two researches, the following conclusions could be derived.

The potato samples originating from Achaia (Greece) simulate with the potato samples irrigated with water containing 100 – 1000 μg L-1 Cr(VI) and Ni (II), while the potato samples originating from Orhomenos (Viotia, Greece, organic farming) and the ones from Naxos (Greece) simulate with the potato samples which were irrigated with water containing 250– 1,000 μg L-1 Cr (VI) and Ni (II) and 250 μg L-1 Cr(VI) and Ni(II), respectively. Furthermore, the potato samples originating from Evia (Greece) appeared to be similar with the potato samples irrigated with water including 100μg L-1 Cr (VI) and Ni (II).  However, the potato samples originating from Cyprus do not simulate with any of the potato samples cultivated in the greenhouse.

The carrot samples originating from Holland (organic farming) simulate with the carrot samples of irrigated water’s concentration about 100μg L-1 of Cr (VI) and Ni (II), whereas the carrot samples originating from Avlona (Greece) simulate with the carrot samples irrigated with water containing 100– 1,000 μg L-1 Cr (VI) and Ni (II). The carrot samples originating from Evia (Greece) and  the ones from Marathon (Greece) simulate with the carrot samples irrigated  with water containing 0 – 250 μg L-1  Cr (VI) and Ni (II) and 100  μg L-1  Cr (VI) and Ni (II),  respectively. Finally, the carrot samples originating from Viotia  (Greece) do not simulate with any of the carrot samples cultivated in the  greenhouse.

Discussion

The results of this study on the carotenoid (lutein and β-carotene) substance and the activity of antioxidant enzymes (catalase and peroxidase) on Cr and Ni treated potatoes and carrots show a clear correlation of Cr and Ni in irrigation water and these secondary metabolites. Moreover, the levels of the same parameters on potato and carrot samples cultivated in areas with water bed pollution simulate the ones on potato and carrot samples irrigated by Cr and Ni solutions. Hence, these secondary metabolites might serve as indicators of heavy metal pollution in water beds and plants.

Given that potatoes and carrots are considered staple foods and they are often used in baby food, contamination by heavy metals of these food tubers not only reduces their nutritional value but also causes a considerable risk. Therefore, legal limits of heavy metals in food need to be revised and introduced by the competent legislative authorities, worldwide.

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